Previous and new PCRs for KHV detection were compared by estimation of their sensitivity in recognizing KHV DNA in plasmids, cell culture extracted KHV DNA and total DNA obtained from field tissue samples. A modified real-time PCR (Gilad et al., 2004), combined with an internal control system (IC2, Hoffmannet al., 2006) in a duplex assay, was used as a “gold standard”. The lowest reliably determined virus concentration between, 5 and 10 KHV DNA genomic equivalents, was found by real-time PCR (Gilad etal., 2004), nested PCR (Bergmann et al., 2006) and one-tube semi-nested PCR. All other published and unpublished PCRs, as well as the commercial Loopamp®, recognized KHV DNA at higher concentrations only. Additionally, KHV variants, newly adapted to European conditions, which could not be detected by PCR according to Bercovier et al. (2005) were found in two field samples from carp and koi from different regions of Germany. A negative influence of sample pooling was shown with field samples tested by real-time PCR.
J Virol Methods. 2010 Feb163(2):229-33. Bergmann SM, Riechardt M, Fichtner D, Lee P, Kempter J. Friedrich-Loeffler-Institut, Institute of Infectology, Federal Research Institute for Animal Health, Südufer 10, 17493 Greifswald-Insel Riems, Germany. sven.bergmann@fli.bund.de |